Université Grenoble Alpes, F-38000 Grenoble, France.
Institute for Advanced Bioscience, INSERM 1209, CNRS UMR 5309, F-38700 La Tronche, France.
Int J Mol Sci. 2022 Jul 21;23(14):8033. doi: 10.3390/ijms23148033.
The group X secreted phospholipase A2 (PLA2G10) is present at high levels in mouse sperm acrosome. The enzyme is secreted during capacitation and amplifies the acrosome reaction and its own secretion via an autocrine loop. PLA2G10 also improves the rate of fertilization. In in vitro fertilization (IVF) experiments, sperm from -deficient mice produces fewer two-cell embryos, and the absence of PLA2G10 is rescued by adding recombinant enzymes. Moreover, wild-type (WT) sperm treated with recombinant PLA2G10 produces more two-cell embryos. The effects of PLA2G10 on mouse fertility are inhibited by sPLA inhibitors and rescued by products of the enzymatic reaction such as free fatty acids, suggesting a role of catalytic activity. However, PLA2G10 also binds to mouse PLA2R1, which may play a role in fertility. To determine the relative contribution of enzymatic activity and PLA2R1 binding in the profertility effect of PLA2G10, we tested H48Q-PLA2G10, a catalytically-inactive mutant of PLA2G10 with low enzymatic activity but high binding properties to PLA2R1. Its effect was tested in various mouse strains, including -deficient mice. H48Q-PLA2G10 did not trigger the acrosome reaction but was as potent as WT-PLA2G10 to improve IVF in inbred C57Bl/6 mice; however, this was not the case in OF1 outbred mice. Using gametes from these mouse strains, the effect of H48Q-PLA2G10 appeared dependent on both spermatozoa and oocytes. Moreover, sperm from C57Bl/6 -deficient mice were less fertile and lowered the profertility effects of H48Q-PLA2G10, which were completely suppressed when sperm and oocytes were collected from -deficient mice. Conversely, the effect of WT-PLA2G10 was not or less sensitive to the absence of PLA2R1, suggesting that the effect of PLA2G10 is polymodal and complex, acting both as an enzyme and a ligand of PLA2R1. This study shows that the action of PLA2G10 on gametes is complex and can simultaneously activate the catalytic pathway and the PLA2R1-dependent receptor pathway. This work also shows for the first time that PLA2G10 binding to gametes' PLA2R1 participates in fertilization optimization.
X 组分泌型磷脂酶 A2(PLA2G10)在小鼠精子顶体中高水平存在。该酶在获能过程中分泌,并通过自分泌环放大顶体反应及其自身的分泌。PLA2G10 还能提高受精率。在体外受精(IVF)实验中,缺乏 PLA2G10 的-/-小鼠的精子产生的二细胞胚胎较少,而添加重组酶可挽救 PLA2G10 的缺乏。此外,用重组 PLA2G10 处理的野生型(WT)精子产生更多的二细胞胚胎。PLA2G10 对小鼠生育能力的影响可被 sPLA 抑制剂抑制,并可被酶反应产物(如游离脂肪酸)挽救,提示其催化活性的作用。然而,PLA2G10 还与小鼠 PLA2R1 结合,这可能在生育能力中发挥作用。为了确定 PLA2G10 的促生育作用中催化活性和 PLA2R1 结合的相对贡献,我们测试了 H48Q-PLA2G10,这是一种催化活性低但与 PLA2R1 结合能力高的 PLA2G10 的突变体。在各种小鼠品系中测试了其作用,包括-/-小鼠。H48Q-PLA2G10 不会触发顶体反应,但与 WT-PLA2G10 一样能有效改善近交 C57Bl/6 小鼠的 IVF;然而,在外交 OF1 小鼠中并非如此。使用这些小鼠品系的配子,H48Q-PLA2G10 的作用似乎取决于精子和卵子。此外,C57Bl/6-/-小鼠的精子生育能力降低,并降低了 H48Q-PLA2G10 的促生育作用,当从-/-小鼠中收集精子和卵子时,这些作用完全被抑制。相反,WT-PLA2G10 的作用对 PLA2R1 的缺失不敏感或较少敏感,提示 PLA2G10 的作用是多模式和复杂的,既作为酶又作为 PLA2R1 的配体。本研究表明,PLA2G10 对配子的作用是复杂的,可同时激活催化途径和 PLA2R1 依赖性受体途径。这项工作还首次表明,PLA2G10 与配子 PLA2R1 的结合参与了受精优化。
Zotero 插件
